Chou Sunwen, Van Wechel Laura C, Lichy Heather M, Marousek Gail I
Medical and Research Services, VA Medical Center and Oregon Health and Science University, P3ID 3710 SW US Veterans Hospital Road, Portland, Oregon 97239, USA.
Antimicrob Agents Chemother. 2005 Jul;49(7):2710-5. doi: 10.1128/AAC.49.7.2710-2715.2005.
A new recombinant phenotyping method was developed for the analysis of drug resistance mutations in human cytomegalovirus (CMV). CMV strain T2211 was derived from strain AD169 by inserting unique restriction sites and a secreted alkaline phosphatase (SEAP) reporter gene for rapid viral quantitation. Specific viral UL97 and pol gene mutations were transferred by recombination into T2211, and their drug resistance phenotypes (for ganciclovir, foscarnet, or cidofovir) were determined by the drug concentrations required to reduce supernatant SEAP activity by 50% (IC50). Changes in the IC50 conferred by the mutations tested (UL97 M460V, C592G, A594V, and L595S and pol del981-2) were similar to those previously reported in marker transfer and conventional plaque reduction assays. The combination of UL97 C592G and pol del981-2 conferred much higher ganciclovir resistance than either mutation alone. The UL97 polymorphism D605E had no measurable effect on ganciclovir susceptibility, alone or in combination with common UL97 resistance mutations. Transfer into strain T2211 facilitates the phenotyping of newly observed mutations, combinations of mutations, and clinical CMV sequences without an accompanying viral isolate.
开发了一种新的重组表型分析方法,用于分析人巨细胞病毒(CMV)中的耐药性突变。CMV毒株T2211由AD169毒株通过插入独特的限制性酶切位点和一个用于快速病毒定量的分泌性碱性磷酸酶(SEAP)报告基因衍生而来。通过重组将特定的病毒UL97和pol基因突变转移到T2211中,并通过使上清液SEAP活性降低50%所需的药物浓度(IC50)来确定其耐药表型(针对更昔洛韦、膦甲酸钠或西多福韦)。所测试的突变(UL97 M460V、C592G、A594V、L595S和pol del981-2)导致的IC50变化与先前在标志物转移和传统蚀斑减少试验中报道的变化相似。UL97 C592G和pol del981-2的组合赋予的更昔洛韦耐药性比单独任何一个突变都高得多。UL97多态性D605E单独或与常见的UL97耐药性突变组合时,对更昔洛韦敏感性均无显著影响。转移到T2211毒株中有助于对新观察到的突变、突变组合以及临床CMV序列进行表型分析,而无需伴随病毒分离株。
